Altering the Modular Architecture of Galectins Affects its Binding with Synthetic α‐Dystroglycan O‐Mannosylated Core M1 Glycoconjugates In situ

Author:

Villones Lareno L.1,Ludwig Anna‐Kristin2,Kikuchi Seiya1,Ochi Rika1,Nishimura Shin‐Ichiro1,Gabius Hans‐Joachim1,Kaltner Herbert2,Hinou Hiroshi1ORCID

Affiliation:

1. Graduate School of Life Science and Faculty of Advanced Life Science Frontier Research Center for Advanced Material & Life Science Hokkaido University N21, W11 Sapporo 001-0021 Japan

2. Physiological Chemistry Department of Veterinary Sciences Faculty of Veterinary Medicine Ludwig-Maximilians-University Munich 82152 MünchenPlanegg-Martinsried Germany

Abstract

AbstractThe multifunctionality of galectins helps regulate a broad range of fundamental cellular processes via cis‐binding and trans‐bridging activities and has gained widespread attention with respect to the importance of the natural specificity/selectivity of this lectin family to its glycoconjugate receptors. Combining galectin (Gal)‐1, −3, −4, and −9 variant test panels, achieved via rational protein engineering, and a synthetic α‐dystroglycan (DG) O‐Mannosylated core M1 glycopeptide library, a detailed comparative analysis was performed, utilizing microarray experiments to delineate the design‐functionality relationships within this lectin family. Enhancement of prototype Gal‐1 and chimera‐type Gal‐3 cis‐binding toward the prepared ligands is possible by transforming these lectins into tandem‐repeat type and prototypes, respectively. Furthermore, Gal‐1 variants demonstrated improved trans‐bridging capabilities between core M1 α‐DG glycopeptides and laminins in microarray, suggesting the possible translational applications of these galectin variants in the treatment of some forms of α‐dystroglycanopathy.

Funder

JKA Foundation

Publisher

Wiley

Subject

Organic Chemistry,Molecular Biology,Molecular Medicine,Biochemistry

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